Searching for just a few words should be enough to get started. If you need to make more complex queries, use the tips below to guide you.
Article type: Research Article
Authors: Lachno, D. Richarda; * | Evert, Barbara A.b | Vanderstichele, Hugoc; 1 | Robertson, Michaelb | DeMattos, Ronald B.d | Konrad, Robert J.d | Talbot, Jayne A.d | Racke, Margaret M.d | Dean, Robert A.d
Affiliations: [a] Eli Lilly and Company, Windlesham, UK | [b] PPD, Richmond, VA, USA | [c] Innogenetics NV, Gent, Belgium | [d] Lilly Research Laboratories, Indianapolis, IN, USA
Correspondence: [*] Correspondence to: Dr. D.R. Lachno, Eli Lilly and Company, Erl Wood Manor, Sunninghill Road, Windlesham, Surrey, GU20 6PH, UK. Tel.: +44 1276 483508; Fax: +44 1276 483416; E-mail: drlachno@lilly.com.
Note: [1] Present address: Biomarkable, Gent, Belgium.
Abstract: The aim of this study was to validate new assays for measurement of amyloid-β (Aβ) peptides in cerebrospinal fluid (CSF) and plasma specimens in clinical studies of solanezumab according to current regulatory recommendations. Four assays based on the INNOTEST® β-AMYLOID(1-42) and prototype INNOTEST β-AMYLOID(1-40) kits were developed and validated. To render these assays ‘solanezumab-tolerant’, excess drug was added to calibrators, quality control, and test samples via a 2-fold dilution with kit diluent. Validation parameters were evaluated by repeated testing of human CSF and EDTA-plasma pools containing solanezumab. Calibration curve correlation coefficients for the four assays were ≥0.9985. Intra- and inter-assay coefficients of variation for Aβ1-40 and Aβ1-42 were ≤13 and ≤15%, respectively for both matrices. Dilutional linearity, within and between assays, was demonstrated for both analytes in CSF and plasma at clinically relevant dilution factors. This dilution regimen was successfully applied during Phase 3 clinical sample analysis. Aβ1-40 and Aβ1-42 were stable in CSF and plasma containing solanezumab at 2–8°C and room temperature for up to 8 h and during 5 additional freeze-thaw cycles from ≤−20 and ≤−70°C. Results of parallel tests on stored clinical samples using INNOTEST methods and proprietary ELISA methods were closely correlated (r2 > 0.9), although bias in reported concentrations was observed between assays. In conclusion, the modified INNOTEST assays provided (relatively) accurate and precise quantification of Aβ1-40 and Aβ1-42 in CSF and plasma containing solanezumab according to established consensus validation criteria. The clinical experience with these assays post validation has shown them to be robust and reliable.
Keywords: Alzheimer's disease, amyloid-β peptide, assay validation, biomarker, cerebrospinal fluid, plasma, solanezumab
DOI: 10.3233/JAD-122317
Journal: Journal of Alzheimer's Disease, vol. 34, no. 4, pp. 897-910, 2013
IOS Press, Inc.
6751 Tepper Drive
Clifton, VA 20124
USA
Tel: +1 703 830 6300
Fax: +1 703 830 2300
sales@iospress.com
For editorial issues, like the status of your submitted paper or proposals, write to editorial@iospress.nl
IOS Press
Nieuwe Hemweg 6B
1013 BG Amsterdam
The Netherlands
Tel: +31 20 688 3355
Fax: +31 20 687 0091
info@iospress.nl
For editorial issues, permissions, book requests, submissions and proceedings, contact the Amsterdam office info@iospress.nl
Inspirees International (China Office)
Ciyunsi Beili 207(CapitaLand), Bld 1, 7-901
100025, Beijing
China
Free service line: 400 661 8717
Fax: +86 10 8446 7947
china@iospress.cn
For editorial issues, like the status of your submitted paper or proposals, write to editorial@iospress.nl
如果您在出版方面需要帮助或有任何建, 件至: editorial@iospress.nl